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Albumin-chaperoned cyanine dye yields superbright NIR-II fluorophore with enhanced pharmacokinetics

机译:白蛋白陪伴的花青染料产生具有增强的药代动力学的超亮NIR-II荧光团

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摘要

NIR-II fluorescence imaging greatly reduces scattering coefficients for nearly all tissue types at long wavelengths, benefiting deep tissue imaging. However, most of the NIR-II fluorophores suffer from low quantum yields and/or short circulation time that limit the quality of NIR-II imaging. Here, we engineered a supramolecular assembly of protein complex with lodged cyanine dyes to produce a brilliant NIR-II fluorophore, providing a NIR-II quantum yield of 21.2% with prolonged circulation time. Computational modeling revealed the mechanism for fluorescence enhancement and identified key parameters governing albumin complex for NIR-II fluorophores. Our complex afforded high-resolution microvessel imaging, with a 3-hour imaging window compared to 2 min for free dye alone. Furthermore, the complexation strategy was applied to an antibody-derived assembly, offering high-contrast tumor imaging without affecting the targeting ability of the antibody. This study provides a facile strategy for producing high-performance NIR-II fluorophores by chaperoning cyanine dyes with functional proteins.
机译:NIR-II荧光成像极大地降低了长波长下几乎所有组织类型的散射系数,有利于深层组织成像。但是,大多数NIR-II荧光团的量子产率低和/或循环时间短,这限制了NIR-II成像的质量。在这里,我们设计了蛋白质复合物的超分子组装体,并结合了花菁染料,以产生出色的NIR-II荧光团,提供了21.2%的NIR-II量子产率,并延长了循环时间。计算模型揭示了荧光增强的机制,并确定了控制NIR-II荧光团白蛋白复合物的关键参数。我们的复合体提供了高分辨率的微血管成像,具有3小时的成像窗口,而游离染料仅需2分钟。此外,将复合策略应用于抗体衍生的装配,可提供高对比度的肿瘤成像,而不会影响抗体的靶向能力。这项研究提供了一种通过用功能蛋白陪伴花青染料来生产高性能NIR-II荧光团的简便策略。

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